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J. Biol. Chem., Vol. 275, Issue 47, 36659-36664, November 24, 2000
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From the Department of Pharmacology, Medical School, University of
Minnesota, Minneapolis, Minnesota 55455-0217
Received for publication, July 28, 2000
Treatment of HEK293 cells expressing the
Prolonged exposure to opioid drugs often produces tolerance,
dependence, and addiction, and the molecular mechanisms underlying these phenomena are still poorly understood. Opioid receptors belong to
the G protein-coupled receptor
(GPCR)1 superfamily (1, 2).
Therefore, one component of opioid tolerance is likely to be mediated
by a phosphorylation-dependent desensitization of the
receptor. Phosphorylation of the prototypic Agonist-induced phosphorylation of opioid receptors has been
demonstrated in different systems (5-10). Concrete demonstration of
the phosphorylation of In light of these discrepancies, it is imperative to identify the
agonist-induced phosphorylation sites and to investigate the role of
the phosphorylation of these sites in the regulation of the Materials--
Dulbecco's modified Eagle's medium and
Geneticin (G418) were purchased from Life Technologies, Inc.
[3H]Diprenorphine (58 Ci/mmol) was supplied by Amersham
Pharmacia Biotech and [32P]orthophosphate (>400 Ci/ml)
by ICN (Costa Mesa, CA). 125I-Acetylated cAMP (2200 Ci/mmol) was purchased from Linco Research Inc. (St. Charles, MO).
Polyclonal antibodies that recognize the acetylated cAMP were purchased
from Calbiochem (La Jolla, CA). NIDA (National Institutes on Health,
Bethesda, MD) supplied the [D-Pen2,5]enkephalin ligand. All other
chemicals were purchased from Sigma.
Generation of the Mutants of the Cell Culture and Transfections--
Human embryonic kidney
HEK293 cells were cultured in minimal essential medium supplemented
with 10% fetal bovine serum, 100 µg/ml streptomycin, 100 IU/ml
penicillin under humidified atmosphere at 5% CO2. Cells
were transiently transfected by the calcium phosphate precipitation
method, and the assays were performed 48 h after transfection.
Pool of stably transfected cells expressing the wild-type or mutant
receptors were isolated in the presence of 1 mg/ml G418, without
selection of individual clones, to avoid any position effect due to the
random integration of each cDNA into the chromosomes. Receptor
expressions were determined by whole cell binding using
[3H]diprenorphine in 25 mM HEPES buffer, pH
7.6. Specific binding is defined as the difference between the
radioactivity bound to the cells in the absence and presence of 100 µM naloxone. HEK293 cells stably expressing the ecdysone
receptor in the pVgRxR vector (EcR-293 cells) were purchased from
Invitrogen and clones stably co-expressing the wild-type or S363A
mutant receptors were described in Ref. 21. 0.2 µM or 2 µM ponasterone A (PA), used to induced respectively low
(0.37 ± 0.14 pmol/mg of protein for the wild-type receptor;
0.14 ± 0.1 pmol/mg of protein for the S363A mutant) or high
(1.03 ± 0.5 pmol/mg of protein for the wild-type receptor; 1.15 ± 0.7 pmol/mg of protein for the S363A mutant) receptor
level, were added 48 h before assays.
Opioid Inhibition of Intracellular cAMP Level--
HEK293 cells
seeded in 100-mm dishes were transiently transfected with 10 µg of
wild-type or mutant receptor cDNAs, as indicated. The next day,
cells were washed, detached, and plated in 24-well plates. Assays were
performed the following day. The cells were pretreated with 1 µM DPDPE for various time intervals (15 min to 6 h),
and were challenged with the same concentration of DPDPE. The
intracellular cAMP level was determined by radioimmunoassay using
125I-acetylated cAMP and rabbit polyclonal antibodies that
recognize the acetylated cAMP, as described in Ref. 10. The amount of cAMP in each well was determined by comparing the ability of the diluted samples to compete for 125I-acetylated cAMP binding
to the antibodies with that of standard concentrations of acetylated cAMP.
Receptor Phosphorylation and Immunodetection--
Transiently or
stably transfected HEK293 cells were seeded in 100-mm dishes, and
proteins were solubilized as described previously in Ref. 10. Briefly,
DOR and mutant receptors were immunoprecipitated using the rat
monoclonal antibody 3F10 (Roche Molecular Biochemicals) and a 60-µl
slurry (50%) of prewashed immunopure protein G-agarose beads (Pierce)
overnight at 4 °C. Receptor proteins were dissociated from the beads
by adding 60 µl of SDS-PAGE sample buffer (62.5 mM Tris
buffer, pH 6.8, 2% SDS, 3 M urea, 10% glycerol, 5%
2-mercaptoethanol, and 0.001% bromphenol blue). The samples were
heated at 42 °C for 1 h and then separated on a 10% SDS-PAGE.
Phosphorylated proteins were visualized and quantified by using the
PhosphorImager Storm 840 system (Molecular Dynamics), and
immunodetections were performed with the peroxidase-conjugated
monoclonal antibodies (12CA5) to the HA epitope tag (Roche Molecular
Biochemicals). Detection was performed using the ECL Plus Western
blotting detection system (Amersham Pharmacia Biotech). Immunoblots
were quantitated by densitometric scanning of film exposed in the
linear range (Molecular Analysis Software, Bio-Rad).
Quantitation of Data Analysis--
Data were analyzed using the GraphPad
program. Mean values from individual treatment groups were
statistically analyzed by a one-way analysis of variance with
subsequent comparisons among treatment groups from their control by
Student's t test.
To investigate the in vivo phosphorylation properties
of DOR, HEK293 cells expressing the wild-type receptor were
radiolabeled with [32P]orthophosphate
(32Pi), then treated with a saturating
concentration (1 µM) of DPDPE, and finally receptors were
immunopurified and analyzed by SDS-PAGE autoradiography (Fig.
1a). Nonspecific signal in
these experiments was negligible (lane 1). In
presence of DPDPE, phosphorylation of the receptor was strongly
stimulated (lane 3) when compared with the basal
phosphorylation in absence of agonist (lane 2) and revealed a diffuse phosphoprotein band migrating at approximately 50-60 kDa, corresponding to that of the HA epitope-tagged DOR (Fig.
1b). Phosphorylation of this protein band was time- and concentration-dependent (data not shown), and the
phosphorylation patterns were similar in HEK293 cells either
transiently or stably expressing the receptor (Figs. 1, 3, and 4).
Additional immunoreactive species were observed in some experiments
with an apparent molecular mass corresponding to the receptor dimers,
consistently with previously described oligomers of DOR (19, 20).
Previous studies suggested that agonist-induced phosphorylation of DOR
occurs at the carboxyl tail domain (11, 12). The intracellular C-tail
of the mouse DOR contains seven Ser and Thr putative phosphorylation
sites (Fig. 2). To identify which Ser and/or Thr are phosphorylated in response to DPDPE, individual or
multiple Ser/Thr were substituted into Ala. All these mutant receptors
were stably expressed in HEK293 cells, and no significant differences
were detected in their ability to bind the antagonist diprenorphine or
the agonist DPDPE, when compared with that of the wild-type receptor
(Table I). Ala substitution of all Ser and Thr at the C-tail of the receptor (mutant DTS) completely blocked
the DPDPE-induced phosphorylation (Fig.
3), indicating that the phosphorylation
site(s) are likely located within the COOH terminus of the receptor. We
systematically substituted all these carboxyl terminus Ser/Thr to Ala.
When compared with the wild-type receptor, the T335A, S344A, T352A, or
T353A mutants did not display any significant differences in
agonist-induced receptor phosphorylation, indicating that none of these
four residues are involved in the DPDPE-induced phosphorylation of the
receptor (Fig. 3, lanes 3-6). In contrast,
mutation of Thr358, Thr361, or
Ser363 to Ala dramatically reduced the phosphorylation
level to about 47.7%, 66.3%, or 91.8%, respectively, as compared
with the wild-type receptor, indicating that these residues are
involved in the agonist-induced phosphorylation of the receptor (Fig.
3). Interestingly, little or no agonist-induced phosphorylation could
be detected with the S363A mutant, indicating that Ser363
is critical for the overall phosphorylation of DOR. The complete blockade of the DPDPE-induced phosphorylation of the receptor by the
S363A mutation (Figs. 3 and 4), suggested
that this residue is either a phosphorylation site or is a kinase
recognition site. The actual phosphorylation of this site was
demonstrated by the mutant receptor in which all the Ser/Thr residues
at the C-tail, except Ser363, were substituted to Ala
(mutant CT/363S, Fig. 4). This mutant showed a significant
agonist-induced phosphorylation and reached 36.6 ± 3.2%
(n = 9) of that of the wild-type receptor. This result showed clearly that Ser363 is the primary phosphorylation
site, and that phosphorylation of DOR could be hierarchical with
Ser363 being the first residue to be phosphorylated.
Hierarchical Phosphorylation of
-Opioid Receptor Regulates
Agonist-induced Receptor Desensitization and Internalization*
,
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-opioid receptor with agonist
[D-Pen2,5]enkephalin (DPDPE) resulted
in the rapid phosphorylation of the receptor. We constructed several
mutants of the potential phosphorylation sites (Ser/Thr) at the
carboxyl tail of the receptor in order to delineate the receptor
phosphorylation sites and the agonist-induced desensitization and
internalization. The Ser and Thr were substituted to alanine, and the
corresponding mutants were transiently and stably expressed in HEK293
cells. We found that only two residues, i.e.
Thr358 and Ser363, were phosphorylated, with
Ser363 being critical for the DPDPE-induced phosphorylation
of the receptor. Furthermore, using alanine and aspartic acid
substitutions, we found that the phosphorylation of the receptor is
hierarchical, with Ser363 as the primary phosphorylation
site. Here, we demonstrated that DPDPE-induced rapid receptor
desensitization, as measured by adenylyl cyclase activity, and receptor
internalization are intimately related to phosphorylation of
Thr358 and Ser363, with Thr358
being involved in the receptor internalization.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
2-adrenergic
receptor by protein kinases, including the G protein-coupled receptor
kinases (GRKs), promotes the association with the receptor of
inhibitory proteins called arrestins (3, 4). This association uncouples
the receptor from the G proteins and promotes targeting of activated
receptors to clathrin-coated pits for subsequent internalization, thus
blunting receptor signaling.
-opioid receptor (DOR) was first reported by
Pei and colleagues (6). Although the sites of
agonist-dependent phosphorylation have not yet been
identified, truncation of the carboxyl tail (C-tail) of DOR showed that
major phosphorylation sites are localized within this domain (11, 12).
Phosphorylation of DOR appears to be the mechanism for agonist-induced
receptor desensitization (6, 13, 14).
[D-Pen2,5]enkephalin (DPDPE)-induced
phosphorylation of DOR seems to involve one or more GRKs (6), and Ala
substitution of the last four carboxyl-terminal Ser and Thr of the
receptor impaired the GRK- and arrestin-mediated receptor
desensitization (13). In Xenopus oocytes, co-expression of
GRK3 and -arrestin2 resulted in an increased rate of
agonist-induced homologous desensitization of DOR (13). However,
truncation of the COOH-terminal 31 amino acids of DOR did not affect
the agonist-induced desensitization of the receptor in CHO cells (15),
unlike what Zhao and colleagues (11) reported in NG108-15 cells. Opioid
receptors are endocytosed in a dynamin-dependent manner by
clathrin-coated pits (14, 16-18). However, the precise role of
phosphorylation in the mechanism of opioid receptor endocytosis is
still not fully understood. A truncated mutant -opioid receptor
undergoes rapid agonist-induced internalization in HEK293 cells, but is
not phosphorylated in the presence of agonist, whereas the same mutant
remained predominantly in the plasma membrane of CHO cells, suggesting
that cell type-specific differences may exist in the biochemical
requirements for the agonist-induced endocytosis (12).
-opioid
receptor. We used series of receptor mutants to identify the
phosphorylation sites at the C-tail of DOR. In this study, we reported
that two sites (Thr358 and Ser363) are
phosphorylated in the presence of DPDPE and, furthermore, that the
phosphorylation of the receptor is hierarchical. Additionally, we
investigated the role played by these two phosphorylation sites in
internalization of the receptor. Here, we also demonstrated that
internalization of the activated receptor plays a role in the loss of
-opioid receptor-mediated inhibition of adenylyl cyclase activity.
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-Opioid Receptor--
The
human influenza virus hemagglutinin (HA) epitope-tagged mouse
-opioid receptor (described in Ref. 19) (Dortag) subcloned into the
expression vector pcDNA3 (Invitrogen, Carlsbad, CA), was used to
generate most of the point mutations. Ser and/or Thr present at the
C-tail of the receptor (from Thr335 to Ser363)
were point-mutated to Ala or Asp by oligonucleotide-directed mutagenesis using a QuickChange site-directed mutagenesis kit from
Stratagene (La Jolla, CA) according to the manufacturer's directions,
except for the following mutants. The T358A, S363A, and S363D mutants
were constructed using the Altered SitesTM in
vitro mutagenesis system provided by Promega Corp. (Madison, WI),
using DOR-1 cDNA subcloned into the phagmid pAlter-1 as template. The nucleotide sequences of all mutants were confirmed by
dideoxynucleotide sequencing using Sequenase II. The
Eco47III-XbaI fragments of the different plasmids
were excised and ligated to the Dortag in pCDNA3 with the same
fragment removed.
-Opioid Receptor Internalization by
Fluorescence Flow Cytometry--
Stably transfected HEK293 cells
expressing wild-type or mutant HA epitope-tagged receptors were treated
with 1 µM DPDPE for the indicated times. Cells were
chilled on ice to stop membrane trafficking, and receptors were
visualized by using a 1:400 dilution of the high affinity mouse
monoclonal anti-HA antibody (HA.11 clone 16B12; Babco, Richmond, CA)
and a 1:500 dilution of the secondary antibodies goat anti-mouse IgG
conjugated with Alexa488 (Molecular Probes, Eugene, OR). Incubations
were performed at 4 °C. Surface receptor staining intensity of
antibody-labeled cells was analyzed using fluorescence flow cytometry
(FACScan, Becton Dickenson, Palo Alto, CA).
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
View larger version (41K):
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Fig. 1.
In vivo DPDPE-induced
phosphorylation of wild-type -opioid
receptor. HEK293 cells transiently transfected with 10 µg of HA
epitope-tagged DOR cDNA or empty vector (mock) were labeled with
32Pi and stimulated with 1 µM
DPDPE for 30 min. The receptors were purified as described under
"Experimental Procedures" and analyzed by phosphorimaging
(a) and immunoblotting (b).
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Fig. 2.
Substitution mutagenesis of the
-opioid receptor C-tail. Potential
phosphorylation sites (Ser/Thr) of the C-tail are indicated in
bold. The numbers above indicate the amino acid
positions in the receptor protein. The amino acid sequences of the
mutants identical to the wild type are represented by dashed
lines, and the changes are as indicated.
Characterization of the -opioid receptor and mutant receptors
lacking putative phosphorylation sites
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Fig. 3.
Analysis of mutant
-opioid receptors DPDPE-dependent
phosphorylation. Cells transiently transfected with 10 µg of
each cDNA were labeled with 32Pi and
stimulated with 1 µM DPDPE for 30 min. a,
extracted phosphoreceptors from wild type and various Ser/Thr mutant
receptors. Pictured is the result of a single experiment representative
of at least three performed. b, receptor proteins detected
by immunoblot of the corresponding phosphorylated gel. c,
receptor phosphorylated bands were quantitatively analyzed with
PhosphorImager, and band intensities were expressed as percentage of
maximal phosphorylation obtained for DOR in presence of 1 µM DPDPE. For each experiment, the amount of
32Pi incorporated into the various receptors
was expressed as a function of the amount of receptor present in each
lane (assessed by densitometric analysis of the immunoblot). Data shown
are means ± S.E.
View larger version (23K):
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Fig. 4.
Hierarchical DPDPE-dependent
phosphorylation of DOR. HEK293 cells stably expressing the wild
type or mutant receptors were labeled, and the ability of 1 µM DPDPE to induce phosphorylation was determined as
described under "Experimental Procedures." Top, amino
acid sequence of the intracellular C-tail of DOR. The different Ala or
Asp substitutions are indicated, and the dashed
lines represent no changes from the wild-type sequence.
Bottom, receptors were purified and resolved on a SDS-PAGE.
After quantification by phosphorimaging and immunoblotting, intensities
of the phosphorylated bands were expressed as a percentage of
DPDPE-induced phosphorylation of the wild-type receptor. Data shown
represent mean ± S.E. of at least three separate experiments.
***, p < 0.001 compared with the phosphorylation
pattern of the S363A mutant.
In order to identify the other phosphorylation sites, Ser363 was mutated to aspartic acid (Fig. 4), which mimics a phosphorylated form of this residue, and which should induce a recovery of the receptor phosphorylation, if the mechanism is hierarchical. As shown in Fig. 4, the S363D mutant restores the DPDPE-induced phosphorylation (compared with the S363A mutant) to about 27.5% of that of the wild-type receptor. This result confirmed, therefore, that Ser363 has to be phosphorylated before another site, and that Thr358 and/or Thr361 is (are) the other phosphorylation site(s). No phosphorylation, however, could be detected with a mutant leaving only Thr361 as a potential phosphorylation site along with the Asp-substituted Ser363 (mutant CT/361T/S363D), suggesting, therefore, that Thr361 is not phosphorylated right after Ser363, but rather Thr358 is. Indeed, the extent of phosphorylation in the T358A mutant is not significantly different (p > 0.1) from the extent of phosphorylation in the mutant leaving Ser363 as the only potential phosphorylation site (mutant CT/363S). Consistently, the lower level of phosphorylation in the S363D mutant (reaching only about 27.5% of that of the wild-type receptor) confirms that only one site is phosphorylated along with Ser363 and that this other residue is Thr358. Nevertheless, the T361A mutation affected the agonist-induced phosphorylation of the receptor. Thr361 could participate in the phosphorylation of the receptor as a kinase recognition/binding site but not as a phosphorylation site. The T361D mutant, which was originally constructed to define the phosphorylation mechanism of DOR, exhibiting almost but not complete recovery of the phosphorylation level as compared with that of the wild-type receptor, might affect to a lesser extent the kinase's recognition/binding to the receptor. This observed recovery was, however, blocked when Ser363 was mutated into Ala along with the T361D substitution (mutant T361D/S363A, Fig. 3), consistently with the critical role of Ser363 in the phosphorylation of the receptor.
Next, we examined the role of phosphorylation in the agonist-induced
desensitization of DOR in HEK293 cells. The kinetics of the loss of
DPDPE inhibition of the adenylyl cyclase activity were monophasic, and
the apparent rate of desensitization was relatively slow, with a
t1/2 of about 1.3 ± 0.25 h
(n = 6, data not shown), consistently with previous study (10). In contrast, DPDPE-induced phosphorylation of the receptor
followed much faster kinetics, showing a maximum within 10 min of DPDPE
exposure (data not shown). The difference in these two rates suggests
that receptor phosphorylation does not directly lead to DOR
desensitization. The failure to correlate phosphorylation to
desensitization of DOR could be due to the relatively high level of
receptor expression (2.2 ± 0.8 pmol/mg of protein) in HEK293
cells. In an earlier study, by controlling the expression level of the
receptor in HEK293 cells with an ecdysone-inducible expression system
(21), we were able to demonstrate that the rate of DOR desensitization
is dependent on the receptor level expressed at the cell surface. Using
the same inducible-expression system to control the expression of the
wild type and S363A mutant receptors, in HEK293 cells (see
"Experimental Procedures"), we could demonstrate that receptor
desensitization kinetics in the presence of DPDPE were receptor
concentration-dependent (Fig. 5). At high levels of receptor
expression (>1 pmol/mg of protein), the desensitization kinetics of
both receptors were relatively slow and indistinguishable, suggesting
that the absence of receptor phosphorylation did not affected the
observed rate of desensitization. Similar results were obtained
when the wild-type receptor and a mutant receptor incapable of being
phosphorylated (mutant T361A/S363A) were transiently expressed in
HEK293 cells (data not shown). At low levels of expression of the wild
type receptor (<300 fmol/mg of protein), when receptor concentration
was limited, the DPDPE-induced loss of response was significantly
faster, and the receptor desensitized completely 40 min following DPDPE
treatment. The elimination of receptor phosphorylation (S363A mutant)
reduced dramatically the extent of desensitization, when expressed at
similar levels as the wild-type receptor. At 40 min following agonist
treatment, 50% of the response remained. Thus, the hierarchical
phosphorylation of DOR at Ser363 is an important but not
obligatory event in the DPDPE-induced desensitization.
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Since internalization is involved in the desensitization of several
GPCRs (4), and since in our earlier study (21) we demonstrated that
receptor internalization also participated in the rapid desensitization
of DOR, we examined whether the DPDPE-induced phosphorylation of
Thr358 and Ser363 would participate in the
agonist-induced receptor internalization. The extent of internalization
of the wild type and mutant receptors from the cell surface were
examined using flow cytometry (Fig. 6).
Kinetics analysis indicated that DOR internalized rapidly in presence
of DPDPE and that about 80% of total cell surface receptor were
internalized in response to 1 h agonist treatment, with a
t1/2 = 10.8 ± 1.6 min (Table II). This rate compared favorably with
previous reports (12, 17, 21). Substitution of the four first Ser or
Thr at the C-tail into Ala (T335A to T353A) did not slow down the rate
or lower the extent of internalization of the corresponding activated receptors. These results suggested, therefore, that none of these four
residues are involved in the DPDPE-induced internalization of the
receptor in HEK293 cells (Table II, group I). In contrast, the DTS
mutant as well as the S363A mutant, both blocking the DPDPE-induced
phosphorylation of the receptor, revealed a substantially slower rate
and lower extent of internalization, strongly suggesting that
phosphorylation of Ser363 and/or Thr358
contributed to the receptor internalization (Fig. 6 and Table II).
Phosphorylation of Ser363 alone (mutant CT/363S) prevented
the receptor from internalizing as efficiently as the wild-type
receptor, suggesting that the phosphorylation of this Ser only is
insufficient to induce receptor internalization. Ala substitution of
Thr358 also blunted the agonist-induced internalization of
the receptor. These results suggest that phosphorylation of
Thr358 is critical for receptor internalization. Indeed,
the S363D mutant (Table II, group I), allowing the DPDPE-induced
phosphorylation of Thr358, exhibited a pattern of receptor
internalization identical to the wild-type receptor. Therefore,
internalization of DOR required the phosphorylation of
Thr358, subsequent to the phosphorylation of
Ser363.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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From our current mutagenesis studies, it is apparent that Ser363 is the primary phosphorylation site, that agonist-induced phosphorylation of DOR occurs in a hierarchical manner, and that Thr358 and Ser363 are the only two residues being phosphorylated. Thr361 participates in receptor phosphorylation, since its substitution into Ala reduced the extent of phosphorylation when compared with the wild-type receptor. Probably, the remaining phosphorylation observed with the T361A mutant comes from Ser363, since Ser363 is phosphorylated independently of Ser/Thr present at the C-tail of the receptor (mutant CT/363S, Fig. 4). Mutation of Thr361 could impair the recognition/binding of a kinase to phosphorylate Thr358, thereby reducing the receptor phosphorylation level. Hierarchical phosphorylation has been demonstrated for only a few GPCRs, including the rhodopsin and the N-formyl peptide receptor (22, 23). Whether this phosphorylation mechanism is conserved among members of the GPCR family, or specific to some of them, remains to be demonstrated. It is possible that phosphorylation of Ser363 creates a new acidic phosphoserine recognition sequence for the subsequent phosphorylation of Thr358 by the same or by another kinase. Several groups have proposed that members of the GRK family can phosphorylate DOR (6, 24). Although the consensus motif of GRK among various GPCRs has not been clearly defined, GRK normally phosphorylate Ser/Thr residues adjacent to an acidic or charged amino acid residue (25). Interestingly, Ser363 and Thr358 are immediately downstream of Pro and Val residues, respectively (Fig. 2). Ser363 is upstream from an aspartic residue, which could serve as a GRK recognition motif. However, Thr358 is upstream from an Ala residue. Whether phosphorylation of Ser363 and Thr358 involved a GRK remains to be demonstrated. Some reports suggested that agonist-induced phosphorylation of the opioid receptors could be mediated by Ca2+/calmodulin-dependent protein kinase II (26), or by mitogen-activated protein kinase (27), but the amino acid motif surrounding Thr358 or Ser363 does not correspond to that of either kinase. Thus, it is tempting to suggest that a yet unknown Ser/Thr kinase is responsible for the DPDPE-induced phosphorylation of DOR. The involvement of this unidentified kinase might be one of the reasons why overexpression of a dominant negative mutant of GRK could not completely block the agonist-induced phosphorylation of the receptor (6, 10).
The rapid and slow desensitization of DOR is dependent on the relative
level of expression of the receptor. The slow rate of a loss of DPDPE
inhibition of forskolin-stimulated adenylyl cyclase in cells expressing
a relatively high level of receptors (Fig. 5) does not correlate with
the rapid DPDPE-induced phosphorylation of the receptor (data not
shown). The relatively high level of receptor expressed at the cell
surface that is not phosphorylated and sufficiently high enough to
maintain the agonist-mediated activity, along with the high efficient
coupling between DOR and the adenylyl cyclase (28), could explain why
the phosphorylation of the receptor did not correlate with the loss of
response. The fact that the mutants showing no detectable
agonist-induced phosphorylation, such as T361A/S363A and S363A mutants
(data not shown and Fig. 5), which exhibit a similar rate and extent of
desensitization as the wild-type receptor at relatively high receptor
levels, suggests that events other than receptor phosphorylation
e.g. internalization/sequestration/down-regulation could be
involved in the slow desensitization of the receptor. At low levels of receptor expression, similar to the levels of expression observed in
endogenously expressing cells, the blockade of the agonist-induced receptor phosphorylation dramatically attenuated the magnitude of rapid
desensitization, implying that the receptor phosphorylation at
Ser363 participates in receptor regulation. Nevertheless,
the ability of the receptor to still desensitize indicates that the
agonist-induced internalization contributes also to the loss of
response, as it was shown for other GPCRs, like for example for the m3
mACh receptor (29) or the µ-opioid receptor (30, 31). We recently
reported that, at low expression levels of µ- and -opioid
receptors, a blockade of receptor internalization leads to a blockade
of the agonist-induced rapid desensitization of these receptors (21, 30). Mutation of Thr358 attenuates the agonist-induced
internalization of DOR, implying that phosphorylation of this residue
is crucial for receptor internalization and hence contributed to the
DPDPE-induced rapid desensitization. Down-regulation of DOR (32, 33),
which involves receptor sequestration and degradation, likely
contributes to the slow loss of receptor activity, regardless of
whether or not the receptor is phosphorylated (Fig. 5).
Thr353 has been reported to be required for the
agonist-induced down-regulation of DOR in CHO cells (34). Since the
DPDPE-induced phosphorylation of DOR in HEK293 cells does not involve
Thr353 (Fig. 3), the ability of the receptor to
down-regulate will not be affected by the inability of the receptor to
be phosphorylated. Similarly, for the µ-opioid receptor, mutation of
Ser363 to Ala attenuated agonist-induced down-regulation
without being an agonist-induced phosphorylation site (35), showing
that phosphorylation of a particular site is not necessarily a signal
for the processing of receptor traffic at the early endosome. Whether
or not Thr353 is involved in DPDPE-induced down-regulation
of the receptor in HEK293 cells remains to be demonstrated, since a
truncated -opioid receptor remaining predominantly in the plasma
membrane of CHO cells, can still internalize in HEK293 cells (12).
Alternatively, a NPXXY motif, common to many GPCRs including
the opioid receptors (36), present at the interface between the seventh
transmembrane and the C-tail of the receptor, or a di-Leu-based motif
(37) present within the third cytoplasmic domain of DOR, could be
implicated in the trafficking of the receptor.
We can propose that phosphorylation of Ser363 will promote
the uncoupling of the activated receptor from its cognate G protein. Then, phosphorylation of Thr358 will regulate
internalization of the receptor, further attenuating receptor-mediated
signaling. Therefore, functional uncoupling of receptor and G protein,
followed by endocytosis, will blunt the response to agonists. Native
opioid peptides or opiate drugs are relatively resistant to proteolytic
degradation in the extracellular environment. Therefore, opioid
receptors may use this regulation mechanism to alter persistent
activation. Whether the same mechanism persists in all in
vitro cell models or in vivo remains to be demonstrated.
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ACKNOWLEDGEMENT |
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We thank Rachid El Kouhen for valuable discussions.
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FOOTNOTES |
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* This work was supported in part by National Institutes of Health Grants DA00564, DA07339, DA01583, DA11806 and the F. and A. Stark Fund of the Minnesota Medical Foundation.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Dept. of Pharmacology,
Medical School, University of Minnesota, 6-120 Jackson Hall, 321 Church
St. S.E., Minneapolis, MN 55455-0217. Tel.: 612-624-6691; Fax:
612-625-8408; E-mail: elkou002@tc.umn.edu.
Published, JBC Papers in Press, September 5, 2000, DOI 10.1074/jbc.M006788200
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ABBREVIATIONS |
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The abbreviations used are:
GPCR, G
protein-coupled receptor;
DOR, -opioid receptor;
GRK, G
protein-coupled receptor kinase;
DPDPE, [D-Pen2,5]enkephalin;
HA, hemagglutinin;
PAGE, polyacrylamide gel electrophoresis;
PA, ponasterone A;
CHO, Chinese hamster ovary.
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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) and S363A (
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were controlled using the ecdysone-inducible expression system as
described previously (